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INTRODUCTION
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We report that in vivo injection of endotoxin (EDTX, 6 mg · kg
1) induces cardiovascular alterations
in rats that closely mimic the clinical situation, as assessed by in vivo hemodynamic measurements in
anesthetized and conscious, chronically instrumented animals. The patch-clamp technique was used
to characterize the L-type calcium current (ICa) and its autonomic regulation in isolated cardiac myocytes. The density of ICa progressively decreased at 12 and 36 h after EDTX injection. However, the
dihydropyridine (±)Bay K 8644 (100 nM) enhanced ICa to levels similar to those in control and EDTX-treated myocytes. In addition, the net stimulatory effect of a 
-adrenergic agonist (isoproterenol) on
ICa was increased 12 h after EDTX injection. This change in the -adrenergic effect declined 24 h
later. The potentiation in the -adrenergic stimulation of ICa was mimicked by L858051 (10 µM), a direct activator of adenylyl cyclase, but not by IBMX (200 µM), a phosphodiesterase inhibitor. Besides,
the antiadrenergic effect of acetylcholine on ICa was unchanged 12 h after EDTX injection, but increased 36 h after EDTX injection. These results support the hypothesis that time-dependent changes in
the adenylyl cyclase pathway in cardiac myocytes may contribute, via the autonomic regulation of
ICa, to the severity of myocardial dysfunction during sepsis.
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INTRODUCTION |
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ABSTRACT
INTRODUCTION
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Septic shock is characterized by a vascular hyporeactivity and a depressed myocardial contraction, both phenomena being largely related to bacterial endotoxin (EDTX) (1). Myocardial dysfunction may result from alterations in calcium homeostasis and/or changes in myofilament properties. The results regarding these cellular functions and their contribution to myocardial depression in sepsis appear contradictory. For instance, the sensitivity of cardiac myofilament to calcium was reported to be unchanged (2) or decreased (3, 4) in cardiac myocytes after EDTX challenge. Furthermore, diastolic and/or systolic intracellular free calcium concentrations were found to be either reduced (2, 5), increased (6), or unchanged (4) on in vivo or in vitro exposure to EDTX or cytokines. Interestingly, the action potential, which determines the amplitude of calcium influx, is shortened in myocytes isolated from endotoxemic animals, as compared with control (5, 7, 8; but see Reference 9). Likewise, both the apparent number of L-type calcium channels (10) and the density of the cardiac L-type calcium current (ICa) (5) are reduced in myocytes isolated from animals treated with EDTX. In addition, ICa is weakened in cardiac myocytes exposed to cytokines in vitro (7, 11).
Transduction pathways are altered in cardiac myocytes
during sepsis or after a prolonged incubation with cytokines.
These include nitric oxide (NO) and cyclic AMP (cAMP)
pathways (7, 11). Sepsis is often accompanied by the induction
of a calcium-independent NO synthase (iNOS or NOS2), but
the role of NOS2 in the myocardial dysfunction during sepsis
remains controversial (7, 11). Concerning the cAMP pathway,
a number of studies examined the effects of proinflammatory
cytokines and/or EDTX on sympathetic and parasympathetic
regulation of cardiac adenylyl cyclase and contraction. In one
in vitro study, the -adrenergic stimulation of adenylyl cyclase
activity was potentiated by proinflammatory cytokines (12)
while in three others it was found to be reduced (7, 13). In addition, the cardiac positive inotropic effects of -adrenergic
agonists was either increased (5, 14), reduced (4, 15), or unchanged (16) during EDTX exposure. The -adrenergic stimulation of ICa was increased (5) or unchanged (9) during sepsis.
Interestingly, adrenergic receptors undergo a biphasic change
after cecal ligation in vivo: an initial increase in the density of
receptors, followed by a reduction due to receptor internalization (17). In addition, sepsis potentiates the inhibitory effect
of the parasympathetic agonist acetylcholine on adenylyl cyclase activity and on the subsequent reduction in cardiac contractility (18, 19).
The above-mentioned studies illustrate some of the mechanisms of cardiac dysfunction that may occur during sepsis, but provide little information on the time course of heart dysfunction during sepsis. Indeed, the development of hypotension is rapid, but multiple organ failure develops more slowly and myocardial dysfunction usually appears 12 to 48 h after the onset of infection and/or bacteremia in humans (20). On the contrary, in the majority of animal studies, myocardial dysfunction takes place on a much faster time scale owing to the administration of large doses of bacterial EDTX. Similarly, incubation or acute administration of high doses of EDTX and/or proinflammatory cytokines can induce functional alterations in isolated myocytes, on a shorter time scale than in the clinical situation (4, 11). Some of the discrepancies found in the literature are likely due to large differences in the protocols used to trigger or mimic sepsis under in vivo and in vitro conditions.
We set up a model of conscious endotoxemic rats that reproduces human hemodynamic alterations. Our aim was to investigate the chronology of the cardiovascular alterations, from the time of intravenous administration of EDTX to the time of the typical cardiovascular dysfunction observed at the peak of sepsis. The chronology of the alterations of isolated cardiac myocytes function was also studied. In line with the aforementioned studies, we have followed up on the amplitude of the L-type calcium current (ICa), the trigger of cardiac contraction, and its regulation by the sympathetic and parasympathetic systems during the development of sepsis.
Part of this work has been published in an abstract form (21).
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In Vivo Experiments
Experiments were performed in male rats (280-320 g) that were given
a 0.3-ml, 1-min injection of either saline or endotoxin (EDTX, 6 mg · kg1, Escherichia coli O111 B4; Sigma, St. Louis, MO) in the dorsal vein of the penis, under brief anesthesia with diethyl ether.* The severity of such a model of unresuscitated, endotoxemic rats was mild.
In a first set of experiments, hemodynamic parameters were measured in rats anesthetized 12 or 36 h after EDTX injection (12-h EDTX and 36-h EDTX rats, respectively). Anesthesia (sodium pentobarbital, 60-100 mg · kg1, administered intraperitoneally) allowed
animal preparation and measurements of arterial pressure and aortic
velocity. In the control group, measurements were also performed at
12 or 36 h after saline injection. However, because there was no difference between the two populations of control rats, their data were
pooled. Hemodynamic parameters were obtained (1) at baseline, 30 min after the stabilization period (that followed the surgery), and (2) after volume loading (saline, 6 ml · kg1, over 5 min) in the three
groups of anesthetized rats (control, 12-h EDTX, and 36-h EDTX), in
order to test the ability of the heart to respond to increased preload.
In the second set of experiments, the effects of EDTX or saline injection were studied in conscious chronically instrumented rats to avoid interference between hemodynamic alterations related to treatment and those related to anesthesia. After instrumentation, rats were allowed to recover for 3 d before intravenous injection. Measurements were performed before and 12, 24, and 36 h after injection of saline or EDTX.
Animal instrumentation. An aortic Doppler probe and carotid arterial catheter were implanted under general anesthesia. After tracheal intubation, rats were mechanically ventilated (tidal volume,
2.5 ml; frequency, 80 cycles · min1) with a ventilator (Harvard pump
683; Harvard Instruments, Boston, MA) at FIO2 equal to 0.5. After
aortic dissection, a 2-mm-diameter silastic cuffed 20-MHz pulsed
Doppler was placed around the ascending aorta. For chronically instrumented animals, the electric wires related to the probes were
brought subcutaneously to the dorsal face of the neck. A heparin-coated polyethylene (PE 50) fluid-filled catheter was also inserted
into the ascending aorta via the right common carotid artery. Its position was checked in postmortem animals. Animal preparation lasted
90-120 min.
Hemodynamic measurement. Aortic velocity was measured by the flow velocity probe connected to a 20-MHz pulsed Doppler flowmeter (engineered by Baylor College of Medicine, Houston, TX). Baseline zero velocity was verified during the diastolic time. This technique allowed continuous measurement of blood flow velocity and its first derivative, the maximal aortic acceleration. Peak values of aortic velocity (Vmax) and acceleration (Gmax) were used as indexes of cardiac performance (22, 23).
Arterial pressure was measured using an arterial catheter connected to a pressure transducer (Abbott Laboratories, Chicago, IL). Data were acquired using data acquisition software (AcqKnowledge, version 3.0; Biopac Systems, Goleta, CA) with a sampling rate of 1,000/s and stored in a Macintosh personal computer. Aortic conductance (Gaor) was calculated as the mean aortic blood flow velocity divided by mean arterial pressure (24). Each data point was the average of 10 consecutive beats recorded in stable condition.
Body weight and temperature were recorded in conscious animals before, 12, and 36 h after EDTX administration. Blood gas analysis and ionic composition, including plasma lactate level, showed no difference among the control and the EDTX animals (data not shown).
Electrophysiology
Myocytes from male rats (180-300 g) were dispersed using collagenase A (0.255 mg · ml1) as described (25). At the end of the perfusion, atria and ventricles were separated, and ventricular myocytes
were resuspended, step by step, in a 1 mM Ca2+-containing solution.
The cells were kept at 37° C until use, within 1-16 h of isolation. 12-h
EDTX and 36-h EDTX myocytes refer to myocytes of rats that received an intravenous injection of EDTX, respectively, 12 and 36 h
before cell isolation whereas control myocytes refer to saline-injected
or untreated animals.
The whole-cell patch-clamp technique was used to record L-type
calcium current (ICa) in Ca2+-tolerant cells; the routine protocol consisted of a test pulse to 0 mV (400-ms duration) elicited every 8 s from
a holding potential of 
50 mV. Occasionally (see Figure 3), the holding potential was increased to 80 mV and the test pulse was preceded by a short pulse to 50 mV (50-ms duration) in the presence of
tetrodotoxin (TTX, 60-90 µM) to inhibit the Na+ current (25). This
protocol minimized the antagonistic effect of (±)Bay K 8644 (see Reference 26). The time-dependent ICa, measured as the difference between the peak inward current during the test pulse and the current at
the end of the pulse (I400), was attributed to the activity of the L-type
calcium channels (25). For the determination of current-voltage relationships for ICa (see Figure 2A) and ICa inactivation curve (data not
shown), a double-pulse voltage-clamp protocol was used (25). Voltage-clamp protocols were generated by a challenger/09-VM programmable function generator (Kinetic Software, Atlanta, GA). The cells
were voltage clamped with a patch-clamp amplified (EPC-7; List,
Darmstadt, Germany). Currents were sampled at a frequency of 10 kHz with a 12-bit analog-to-digital converter (DT2827; Data Translation, Marlboro, MA) connected to a PC-compatible computer. The
experiments were performed at room temperature (24-32° C), and in
a given experiment, the temperature did not change by > 2° C.
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Solutions. The external Cs+-containing solution contained 107 mM
NaCl, 10 mM HEPES, 20 mM CsCl, 4 mM NaHCO3, 0.8 mM NaH2PO4, 1.8 mM MgCl2, 1.8 mM CaCl2, 5 mM D-glucose, 5 mM sodium pyruvate, 6-9 × 104 mM TTX (pH 7.4, adjusted with CsOH). External solutions were applied as described (27). The patch pipettes (0.5-1.0
M
) were filled with an internal Cs+-containing solution composed of
119.8 mM CsCl, 5 mM EGTA (acid form), 0.062 mM CaCl2 (pCa
8.5), 4 mM MgCl2, 5 mM disodium phosphocreatine, 3.1 mM
Na2ATP, 0.42 mM Na2GTP, 10 mM HEPES (pHN 7.3 adjusted with CsOH).
Drugs. Collagenase was from Boehringer GmbH (Mannheim, Germany). Tetrodotoxin was from Latoxan (Rosans, France). L855081
(Calbiochem, La Jolla, CA) was dissolved in distilled water at 10 mM
and stored at 20° C until single use. All other drugs were from Sigma.
Nifedipine and (±)Bay K 8644 were dissolved in ethanol at 1 mM, and
stored at 20° C until single use. Drug-containing solutions were prepared at the beginning of each experiment.
Data analysis. During patch-clamp experiments, the maximal amplitude of whole-cell ICa was measured as previously described (25). Membrane capacitances were calculated as described by Scamps and co-workers (25). On-line analysis of the recordings was made possible by programming a PC-compatible computer in Assembly language (Borland) to determine, for each depolarization, peak and steady state current values, as well as the time to peak and the integral of ICa (27). Here, the "basal" condition for ICa refers to the absence of cAMP- elevating agents.
Mean maximal effects (Emax) and half-maximal concentrations (EC50) were obtained by fitting sets of individuals values to the Michaelis-Menten equation. Correlation coefficients were found to be > 0.95 for the curves presented in Figures 4 and 6.
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Statistical Analysis
Results are expressed as means ± SEM. When appropriate, statistical comparisons of two groups of data were made with a Student t test. Comparisons among the three groups (control, 12-h EDTX, and 36-h EDTX) were made using analysis of variance (ANOVA)-factorial or ANOVA-two way for repeated measures.
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EDTX-induced Hemodynamic Alterations In Vivo
Table 1 shows that in vivo injection of EDTX consistently increased body temperature and decreased body weight, as reported in other animal studies (7). The mortality rate was 5%
over the 36 h after EDTX administration. Hemodynamic consequences of EDTX injection in vivo, studied in anesthetized
animals, showed a dominant vascular dysfunction 12 h after
EDTX administration and a time-dependent impairment in
cardiac function over the 36 h. In the 12-h EDTX group, the
large vasodilation (a two-fold increase in Gaor compared with
control) induced a decrease in systolic arterial pressure (SAP,
25 ± 3% of control, p < 0.05, Table 1) that was partially
compensated by volume loading. The indexes of cardiac performance, Vmax and Gmax, were slightly diminished after EDTX
administration (10 and 15% of control, respectively) but
were greatly improved by volume loading (Figure 1). Thus the moderate alteration in cardiac performance, likely compensated by the associated decrease in afterload, properly responded to volume loading in 12-h EDTX animals.
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Similarly, 36-h EDTX rats had a decreased SAP, as compared with control animals. However, both Vmax and Gmax became much more depressed in 36-h EDTX than in control and 12-h EDTX rats. In addition, these indexes of cardiac performance remained unresponsive to volume loading (Figure 1). Accordingly, these data indicate a greater alteration of heart function in 36-h EDTX than in 12-h EDTX rats.
Because anesthesia can distort in vivo measurements in an
unpredictable manner (28), we repeated these measurements
in conscious, chronically instrumented rats (Figure 1C). Although the amplitudes of Vmax and Gmax were ~ 25 to 30%
higher in awake compared with anesthetized animals, EDTX
was found to exert similar hemodynamic effects. Vmax and
Gmax remained stable in awake control rats whereas EDTX
treatment induced a time-dependent decrease in Vmax and
Gmax (respectively, 30 and 35% versus control at 36 h). Alterations in SAP and aortic conductance after saline or EDTX
administration were similar in conscious rats to that observed
in anesthetized rats (Table 2). Thus, these data show that myocardial dysfunction was present in all EDTX-treated rats, regardless of anesthesia.
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In Vivo Treatment with EDTX Reduces ICa in Isolated Ventricular Myocytes
By using a routine protocol wherein the cardiac L-type calcium current (ICa) was elicited at 0 mV, we found that the amplitude of ICa (814.7 ± 28.2 pA in control cells, n = 161) tended to be lower in myocytes isolated from 12-h EDTX rats (772.0 ± 36.3 pA, n = 74), and in myocytes from 36-h EDTX rats (665.9 ± 25.4 pA, n = 99; p < 0.01 versus control and 12-h EDTX rats). Cell-to-cell variability was minimized by normalizing the amplitude of ICa to cell membrane capacitance (Cm), an estimate of cell membrane area. The density of ICa (ICa/Cm) was lower in 12-h EDTX myocytes than in control cells (respectively, 5.04 ± 0.20 and 5.90 ± 0.15 pA/pF, n = 70 and 159, p < 0.001; Figure 2A). The density of ICa was even lower in 36-h EDTX myocytes (4.41 ± 0.14 pA/pF, n = 95, p < 0.001 versus control and p < 0.01 versus 12-h EDTX). L-type calcium channels being voltage dependent, their behavior was examined at different membrane potentials (Figure 2B). ICa was reduced in a uniform manner at every potential in 12-h EDTX and 36-h EDTX myocytes, as compared with control cells. Membrane integrity was not affected by EDTX treatment because the "leak current" (i.e., the current measured at the end of the pulse, I400) was similar in the three groups of cells.
The reduction in ICa may be explained by an increase in the inactivation rate of the calcium channels. However, an index of the course of ICa inactivation, the ratio of ICa time integral over peak ICa density (29), was unchanged in EDTX myocytes (30.90 ± 0.65 ms in control, n = 96, 29.91 ± 0.91 ms in 12-h EDTX, n = 34, 29.76 ± 0.70 ms in 36-h EDTX, n = 65). Furthermore, the time to peak, the steady state inactivation curves, and the current-frequency relationships of ICa (in the 0.125- to 2-Hz range) were similar in the three groups of cells (data not shown). Thus, the reduction in ICa observed in EDTX myocytes was likely due to a reduction in the number of functional calcium channels, with no modifications in the gating properties of individual channels.
Effects of Dihydropyridine Agonists and Antagonists on ICa
Nifedipine (0.5 µM), a dihydropyridine receptor antagonist that selectively blocks L-type calcium channels (25, 26), inhibited most of the macroscopic ICa (93.6 ± 3.2%, n = 7) in control myocytes. The inhibitory effect of nifedipine (0.5 µM) was similar in 12-h EDTX (92.1 ± 2.0%, n = 8) and 36-h EDTX myocytes (91.1 ± 1.9%, n = 7) as compared with control. Hence, ICa was carried by the same type of channels in all groups of cells.
(±)Bay K 8644, a dihydropyridine agonist, enhanced ICa density to the same level in control and EDTX myocytes (Figure 3). The mean stimulatory effect of (±)Bay K 8644 on ICa was much larger in 12-h EDTX and 36-h EDTX myocytes (350.5 ± 44.44 and 322.4 ± 15.4% of basal, respectively) as compared with control (232.0 ± 9.3% of basal, p < 0.01 and p < 0.001 versus 12-h EDTX and 36-h EDTX, respectively). Because the macroscopic properties of ICa were not changed in EDTX myocytes, as compared with control (see above), (±)Bay K 8644 appeared to "mobilize" calcium channels made unavailable by the in vivo injection of EDTX.
Stimulation of ICa by the -Adrenergic
Agonist Isoproterenol
-Adrenergic agonists, such as isoproterenol (Iso), produce a
well-documented stimulation of ICa (26). In the presence of Iso (10 nM and 1 µM), ICa density was somewhat higher in 12-h EDTX myocytes as compared with control and 36-h EDTX
myocytes (Figure 4A). Indeed, the net stimulatory effect of
Iso (i.e., Iso-stimulated ICa basal ICa) was larger in 12-h
EDTX myocytes (+7.9 ± 0.7 pA/pF with 10 nM Iso, and +9.7 ± 1.0 pA/pF with 1 µM Iso) than in control cells (+5.6 ± 0.4 pA/
pF with 10 nM Iso, and +7.1 ± 0.6 pA/pF with 1 µM Iso; respectively, p < 0.01 and p < 0.05 versus 12-h EDTX). However, the net effect of Iso declined in 36-h EDTX myocytes
(+5.1 ± 0.3 pA/pF with 10 nM Iso, and +6.36 ± 0.6 pA/pF
with 1 µM Iso; respectively, p < 0.005 and p < 0.01 versus 12-h
EDTX). Interestingly, the net stimulatory effect of Iso was as
large in control as in 36-h EDTX myocytes, although the basal
ICa was much lower in 36-h EDTX myocytes.
The -adrenergic regulation of ICa was studied over a wider
range of Iso concentrations. To resolve the changes in the
-adrenergic pathway, the Iso-stimulated ICa was normalized
to the amplitude of the basal ICa, as summarized in Figure 4B.
The stimulatory effect of Iso on ICa was significantly scaled up
in 12-h EDTX myocytes as compared with control, over the
whole range of concentrations. The stimulatory effect of Iso
was also enhanced in 36-h EDTX myocytes as compared with
control, but only in the 0.1-1 µM range. The dose-response
curve for Iso appeared shifted to the right in 36-h EDTX myocytes, as compared with 12-h EDTX myocytes. Thus the
change in the -adrenergic stimulation of ICa appeared more
beneficial in 12-h EDTX than in 36-h EDTX myocytes, especially at low concentrations of Iso. The -adrenergic agonist
seemed to "mobilize" voltage-reluctant calcium channels in
EDTX myocytes, and this effect can be demonstrated at maximal concentrations of Iso. We next investigated the mechanism accounting for the increase in the maximal effect of Iso
in EDTX myocytes.
Effect of the Cyclic AMP Pathway on ICa
-Adrenergic receptor density undergoes a biphasic change
during sepsis in rat hearts (17). To examine whether changes
in -adrenergic receptors account for the modifications in the
effects of Iso on ICa, we first studied the effect of an adenylyl
cyclase activator, the forskolin analog L858051, which bypasses -adrenergic receptors (30). As illustrated in Figure
5A, 10 µM L858051 induced a twofold increase in basal ICa in
control myocytes, and a threefold increase in myocytes isolated from both 12-h EDTX and 36-h EDTX-treated rats.
Thus, the maximal effect of L858051 on ICa was comparable to
the maximal effect of Iso. Hence, a modification in -adrenergic receptor density does not account for the enhancement of
the -adrenergic stimulation of ICa in EDTX myocytes.
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The regulation of ICa in EDTX-treated rats appeared to be modified at steps located downstream from cAMP production. One such mechanism could be the cAMP-dependent protein kinase (cA-PK) Because an enhanced activity of cA-PK has been reported in an animal model of sepsis (31). Therefore, we examined the effect of a phosphodiesterase inhibitor (3-isobutyl-1-methylxanthine, IBMX) that elevates cAMP levels by inhibiting cAMP hydrolysis. As illustrated in Figure 5B, a saturating concentration of IBMX (200 µM) induced a twofold increase in basal ICa in control myocytes as well as in myocytes derived from EDTX-treated rats, both after 12 and 36 h of in vivo treatment. Thus, in the absence of a stimulation of cAMP production, the stimulatory effect of cAMP accumulation on ICa is not modified in EDTX myocytes, as compared with control.
Muscarinic Regulation of ICa
Acetylcholine (ACh), the main neurotransmitter of the parasympathetic system, counteracts the effects of -adrenergic
agonists in vivo, and antagonizes the -adrenergic stimulation
of ICa in isolated myocytes (32). This antiadrenergic effect of
ACh on ICa was first studied in the continuing presence of 10 nM Iso (Figure 6A). The density of the Iso-stimulated ICa was
reduced to the same extent by ACh (3 µM) in control and 12-h
EDTX myocytes. The density of ICa was much lower in 36-h
EDTX myocytes, in the absence and in the presence of ACh.
In these cells, the Iso-stimulated ICa was reduced almost to the
basal level by the muscarinic agonist. The inhibitory effect of
ACh was then normalized to the net stimulatory effect of Iso,
and further examined at different concentrations of ACh (Figure 6B). The maximal inhibitory effect of ACh was significantly increased in 36-h EDTX myocytes (79.4 ± 13.1% inhibition of the Iso stimulation, n = 8), as compared with control
and 12-h EDTX myocytes (respectively, 56.0 ± 3.9 and 51.5 ± 4.1% inhibition, n = 10 and n = 6, both p < 0.05 versus 36-h
EDTX). Thus, in 36-h EDTX myocytes, the low density of ICa
in the presence of Iso plus ACh was not only due to the low
density of the Iso-stimulated ICa, but also to an enhanced effect of ACh.
The effect of ACh was also studied in the presence of 1 µM
Iso, a concentration at which the -adrenergic stimulation was modified not only in 12-h EDTX myocytes, but also in 36-h
EDTX myocytes (see above). Under this condition, the antiadrenergic effect of ACh was again similar in control and 12-h
EDTX myocytes, and the maximal effect of ACh in 36-h
EDTX myocytes was enhanced as compared with control
(data not shown). Overall, the in vivo treatment with EDTX
induces an increase in the inhibitory effect of ACh. This phenomenon was delayed as compared with the changes in the
-adrenergic regulation of ICa. The next experiments were aimed at illustrating the mechanisms involved in this alteration in the muscarinic regulation.
Muscarinic Regulation of the Cyclic AMP-dependent Stimulation of ICa
The maximal effect of ACh (3 µM) ICa was examined in the
presence of L858051 (Figure 7A). In vivo treatment with
EDTX potentiated the ACh inhibition of the L858051-stimulated ICa, an effect that was clearly significant in 36-h EDTX
myocytes. These results suggest that -adrenergic receptors,
and/or their coupling efficiency to adenylyl cyclase, are not the
primary components responsible for the alteration of the response of ICa to Iso and ACh in EDTX-treated rats.
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The IBMX-stimulated ICa was also reduced in a reversible manner on application of ACh in control and EDTX myocytes (Figure 7B). Interestingly, the maximal inhibitory effect of ACh (10 µM) on ICa, observed in the presence of IBMX, was identical in the control and EDTX myocytes. Thus, the muscarinic regulation of ICa was not modified when cAMP level was elevated by phosphodiesterase inhibition. Altogether, the in vivo treatment with EDTX does not affect the cAMP-dependent regulation of ICa at a step located downstream from cAMP production.
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We found that a single in vivo administration of EDTX induces time-dependent changes in rat cardiovascular function
that mimic the clinical situation. At the cellular level, EDTX
injection induced a decrease in the basal density of ICa in isolated rat ventricular myocytes. The autonomic control of ICa
was also modified in a time-dependent manner after EDTX
challenge. The -adrenergic stimulation of ICa was potentiated
at 12 h and to a lesser extent at 36 h after EDTX injection,
whereas the antiadrenergic effect of ACh on ICa was unchanged at 12 h, but strongly increased at the late stage of sepsis. Our findings support the view that sepsis induces a remodeling of the autonomic control of cardiac function.
Septic shock is characterized by hypotension and a low cardiac index in patients before resuscitation. At the early stage of sepsis, fluid resuscitation increases the cardiac index to a normal level or even to a level greater than before sepsis (33). Some patients progress to a more serious cardiac dysfunction and become unresponsive to the usual treatment, including fluid resuscitation and even catecholamine administration (15). In our study, EDTX administration in awake rats induced similar hemodynamic changes and appeared to mimic the cardiovascular dysfunction observed in septic patients.
In vivo injection of EDTX induced a progressive decline in the density of ICa. Zhong and colleagues (5) also reported a slight slowing of the decay of ICa, related to a drastic (~ 50%) reduction in ICa. The lack of modification in the kinetics of ICa in the present study is probably related to a smaller reduction (~ 25%) in ICa density. The other properties of ICa were unaffected by EDTX treatment (voltage dependency, steady state inactivation). Furthermore, in myocytes from EDTX-treated rats, ICa was sensitive to concentrations of nifedipine and (±)Bay K 8644 known to be selective for the L-type calcium channels. These data demonstrated that ICa was carried by L-type Ca2+ channels in EDTX myocytes.
The decline in basal ICa may participate in the myocardial dysfunction during sepsis. First, EDTX injection was reported to shorten the cardiac action potential (5, 30; but see Reference 9). Second, the maximal rate of cell shortening and the rise in intracellular calcium were shown to be considerably reduced in EDTX myocytes (5, 30). Because ICa is the trigger of cardiac contraction, a reduction in the density of ICa is likely to exert significant effects on the contraction in EDTX myocytes. Importantly, sarcoplasmic reticulum is unlikely to balance the reduction in ICa because it was found to be essentially unaffected during sepsis (8). However, the decrease in cardiac myofilament response to calcium (3, 4) might aggravate further the consequences of a reduced calcium influx in cardiac myocytes during sepsis.
The mechanism of ICa reduction remains unclear. The simplest explanation for this reduction is a diminution in the total number of calcium channels, as already reported in hearts of endotoxemic rabbits (10), with no modification in the voltage-dependent properties of the remaining functional channels. However, this hypothesis is difficult to reconcile with the results obtained with (±)Bay K 8644 (and with Iso; see below). Indeed, the dihydropyridine agonist had a more pronounced stimulatory effect on ICa density in 12-h EDTX and 36-h EDTX myocytes as compared with control myocytes, thereby canceling the differences in ICa density between the three groups of cells. Because the voltage-dependent properties of ICa in the presence of (±)Bay K 8644 were not different in EDTX and control myocytes (data not shown), it looks as if (±)Bay K 8644 increased the number of functional calcium channels, which contradicts its well-established mode of action (26). Further experiments are needed to understand the mechanism of ICa reduction by EDTX and the "mobilizing" effect of (±)Bay K 8644.
The -adrenergic stimulation of ICa increased 12 h after
EDTX injection in the rat. A similar finding was obtained in
guinea pig hearts as early as 4 h after EDTX injection (5). We
show that the dose response to Iso was scaled up at this early
stage of sepsis in the rat. These findings might explain the increased positive inotropic effect of Iso observed early after
EDTX injection in guinea pig [after 4 h (14)] and rat heart [after 6 h (16)]. In addition, the antiadrenergic effect of ACh on
ICa was unaltered in 12-h EDTX myocytes. Thus, parasympathetic activity may be unable to counteract an increase in the
cardiotonic effect of sympathetic activity, at the level of the
cardiac myocyte. However, EDTX injection induced further
changes because, in 36-h EDTX myocytes, (1) the effect of Iso
on ICa was somewhat attenuated, with a reduction in the apparent sensitivity to the -adrenergic agonist, and, more importantly, (2) the antiadrenergic effect of ACh was increased, owing to a larger maximal effect of the muscarinic agonist.
These results could provide a cellular mechanism for either
(or both) the increased negative inotropic effect of muscarinic
agonists observed during sepsis (18, 19), and the impaired
-adrenergic stimulation by dobutamine in late and severe
sepsis in humans (15). Overall, contradictory reports on the
effects of -adrenergic agonists during sepsis might be due to
the fact that the cardiac preparations used were engaged at
different stages of the septic process.
In light of the multiple biochemical changes occurring during sepsis (7), more than a single step in the cAMP cascade
might contribute to the remodeling of the autonomic regulation of ICa. The experiments with Iso and L858051 demonstrated that alterations were taking place at the level of adenylyl cyclase and/or cAMP hydrolysis by phosphodiesterases.
Importantly, the regulation of ICa was identical in control and
EDTX myocytes in the presence of IBMX. Thus, a modification at a step beyond cA-PK cannot explain the effects of Iso
and ACh on ICa in EDTX myocytes. Accordingly, the sensitivity of the calcium channels toward cA-PK was not significantly modified by the EDTX challenge. In addition, a change in
phosphodiesterase activity alone is also unlikely to account
for the effects of EDTX treatment. Indeed, the extent of the
-adrenergic stimulation in EDTX myocytes (~ 260% of the
basal ICa) cannot be reached in control myocytes, even in the
presence of IBMX plus Iso (data not shown). An attractive
hypothesis is that EDTX injection induces a hyperdynamic
state of adenylyl cyclase. A somewhat similar finding was obtained previously with an in vitro application of TNF-
(12), a
cytokine known to participate in septic shock (7). In this
study, the stimulatory effects of forskolin or the stimulatory G
protein (Gs) on cardiac adenylyl cyclase was increased on prolonged exposure to the cytokine (12). After this initial increase in efficacy of Iso observed at 12 h, the potency of the
-adrenergic agonist to stimulate ICa was markedly reduced 24 h later. A progressive reduction in the number of -adrenergic
receptors could account for this observation. -Adrenergic receptors are indeed enrolled into an internalization process
during the last phase of sepsis (17). This phenomenon may be
a consequence of the presence of high levels of circulating catecholamines and/or exaggerated in situ sympathetic stimulation (1, 7, 15). Interestingly, both circumstances also increased
the expression of inhibitory G proteins (Gi) (7), which might
contribute to the increase in the muscarinic inhibition of ICa
observed in 36-h EDTX myocytes.
In conclusion, a decrease in ICa may be involved in the myocardial dysfunction occurring during septic shock. This alteration in ICa appeared to be compensated by an early potentiation of the -adrenergic response. However, this putative
compensatory mechanism was not sustained. It was challenged
by an increase in the muscarinic response, which seemed to
dominate at the late stage of sepsis, when cardiac dysfunction
takes place. Overall, our study does not support the view than
the myocardial depression is due to a single predominant biochemical change. Instead, sepsis appears to induce a remodeling of multiple cardiac functions, the balance of which might
contribute to the severity of the myocardial dysfunction.
| |
Footnotes |
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Correspondence and requests for reprints should be addressed to Pierre-François Méry, INSERM U-446, Laboratoire de Cardiologie Cellulaire et Moléculaire, Université de Paris-Sud, Faculté de Pharmacie, 5, rue Jean-Baptiste Clément, F-92296 Châtenay-Malabry Cedex, France. E-mail: Pierre.Francois{at}cep.u-psud.fr
(Received in original form August 28, 1998 and in revised form March 2, 1999).
* The investigation conforms with the European Community guiding principles in the care and use of animals (86/609/CEE, CE Off. J. L358, December 18, 1986) and the French decree 87/748 of October 19, 1987 ( J. Off. République Française, October 20, 1987, pp. 12245-12248). Authorizations to perform animal experiments according to this decree were obtained from the French Ministère de l'Agriculture et de la Forêt (04226, April 12, 1991).Acknowledgments: The authors thank Patrick Lechêne for skillful technical assistance, Florence Lefebvre for preparation of the cells, and Françoise Boussac for editorial help. The authors also thank Jacqueline Hoerter and Philippe Mateo for their involvement in pilot experiments, as well as Thomas Eschenhagen, Dan Longrois, and Frédérique Scamps for helpful discussions.
Supported by grants from the Société de Réanimation de Langue Française, Fondation de France, The Ministère de l'Enseignement Supérieur et de la Recherche (DSPT5), and the Direction de la Recherche Clinique, AP-HP and the Société de Réanimation de Langue Française. Najah Abi-Gerges was a recipient of a fellowship from the Fondation pour la Recherche Médicale. Benoit Tavernier was a recipient of a fellowship of the Institut Electricité-Santé, and from the Société Française d'Anesthésie-Réanimation.
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References |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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